Corynebacterium diphtheriae MLST Protocol

Genes

The Corynebacterium diphtheriae MLST scheme uses fragments of the following seven house-keeping genes:

ATP synthase alpha chain (atpA)
DNA polymerase III alpha subunit (dnaE)
Chaperone protein (dnaK)
Elongation factor G (fusA)
2-isopropylmalate synthase (leuA)
2-oxoglutarate dehydrogenase E1 and E2 components (odhA)
DNA-directed RNA polymerase beta chain (rpoB)

PCR amplification

Reaction conditions for all the primers were as follows: initial denaturation at 96°C for 1 min; 35 cycles of denaturation at 96°C for 1 min, primer annealing at 58°C for 1 min, extension at 72°C for 2 min; followed by a final extension step of 72°C for 5 min. Each 25 µl amplification reaction mixture comprised: 5 µl Q solution (Qiagen), 3.0 µl chromosomal DNA (5-20 ng/µl), 1.0 µl forward primer (10 pmol/µl), 1.0 µl reverse primer (10 pmol/µl), 5.0 µl 10x PCR buffer (Qiagen, contains 15 mM MgCl2), 0.5 µl dNTP solution (Qiagen, 10 mM each dNTP), 0.125 µl Taq polymerase (Qiagen, 5units/µl), 0.5 µl of MgCl2 (25mM) and 25.75 µl PCR-grade water. All Qiagen solutions from PCR CORE Kit (Cat No. 201225). The amplification product was then purified using MinElute UF plates (Qiagen) following the manufacturers protocol before being used in a sequencing reaction. Sequencing was carried out on each DNA strand with BigDye Terminator Ready Reaction Mix v3.1 (PE Biosystems, Foster City, US) under standard sequencing conditions according to the manufacturer's protocol. Unincorporated dye terminators were removed by precipitation with 95% alcohol. The reaction products were separated and detected on an ABI PRISM genetic analyser 3100 (PE Biosystems) using a standard sequencing module with a Performance Optimised Polymer and 5 cm array. The primers used in MLST analysis of C. diphtheriae are listed below. Note the rpoB sequencing primers were described by Khamis et al. 2004 J Clin Microbiol 42:3925-3931.

Gene Direction Primer Sequence
atpA F GCGATTGCGAACTACACC
R CTCGAGGAATACCTRACC
dnaE F TGCGTCATCTGATTGAAA
R CGGTCCAATAAGACACCA
dnaK F ACTTGGGTGGCGGTACTT
R TGGTGAACGTCTCGGAAC
fusA F TACCGCGAGAAGCTCGTT
R GAAGGTTGGGTCCTCTTC
leuA F CGTGCACTTCTACAACTC
R ACCGTGATCGGTCTTCAT
odhA F CGGCAAGGAAASCATGAC
R GTTGTCGCCRAACATCTG
rpoB F AAGCGCAAGATCCAGGAC
R TCGAACTCGTCGTCATCC

 

Sequencing

Gene Direction Primer Sequence Allele size (bp)
atpA F AGAAGGCGACGAAGTMAAGC 378
R CRGAATCAGAAGCTGGWGCA
dnaE F GTGCGACAAGCTGGTGTG 354
R GGCTTWCGGCCATTYTTG
dnaK F AGATGGCTATGCAGCGTCT 345
R GATGAGCTTGGTCATCACG
fusA F CGTAAGCTGACCGTTAACTC 360
R CCATGGACTCRAGGATGA
leuA F CCYATCATCATCAAYCTGCC 384
R CAGCTGGTTGCAGTAYTC
odhA F TBCAAGATCGCATYGARRC 381
R TWGGCTCGATGTGKCCTTC
rpoB F CGWATGAACATYGGBCAGGT 342
R TCCATYTCRCCRAARCGCTG